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Re: [ccp4bb] Tag, you're in! Flag, V5, etc
 

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Subject: Re: Tag, you're in! Flag, V5, etc
From: Chun Luo chun {- at -} ACCELAGEN {- dot -} COM
Date: 2008-02-08
Yongfu,



Small peptide tags usually don't interfere with protein folding and linker
is not required. With removable tags, the protease site also serves as a
linker. In most cases, putting a protease cleavage site such as TEV or
PreScission site is good enough. The proteases (HRV3C and TurboTEV) are now
available at a cost less than using thrombin
(http://www.accelagen.com/proteins.htm#protease). So you can remove the tag
and the proteases easily.



For detection with Western blot, Flag, HA, Myc-tags are good and His-tag may
be problematic since not all anti-His antibodies work well. However, His-tag
gives an option to do binding in denatured condition. So for purification
purpose, His-tag is probably your best bet.



If you know that the precise N- or C-terminus is critical for protein
function, put the tag on the other end or use Factor Xa cleavage site to
remove N-terminal tag. You'll be surprised to find out that many proteins
can be easily purified without using any tag. When we did the purification
of SARS 3C protease, the purification scheme without using tag was actually
simpler with higher yield. We have purified proteins for crystallography
without using affinity tag from insect cells at an expression level of ~1
mg/L. From E. coli, a 3-step purification is generally sufficient to purify
protein without using affinity tag.



Chun



Chun Luo, Ph.D.
The Protein Expert
Accelagen, Inc.
11585 Sorrento Valley Road, Suite 107
San Diego, CA 92121
TeL: 858-350-8085 ext 111
Fax: 858-350-8001
chun@accelagen.com
www.accelagen.com







_____

From: CCP4 bulletin board [mailto:CCP4BB@JISCMAIL.AC.UK] On Behalf Of Y. -F.
Li
Sent: Thursday, February 07, 2008 1:29 PM
To: CCP4BB@JISCMAIL.AC.UK
Subject: [ccp4bb] Tag, you're in! Flag, V5, etc



Hello,



I'd appreciate it if anyone could provide information (experiences or
publications) on the following:



1. Put a tag such as FLAG, V5, etc etc, at the N- and/or C-termini, in order
for specific detection, but not interfering with protein folding/structure;

2. Is a linker between the tag and target protein needed? What linkers
(length, specific sequences) would you suggest?

3. What are the choices of such tags and why would you recommend them?



Thank you for your time and sharing in advance.



Yongfu Li
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